Objective: To investigate the binding capacities of differently glycosylated IgA1 on human umbilical vein endothelial cells (HUVEC).
Methods: Serum IgA1 was purified by jacalin affinity chromatography and then was desialylated and/or degalactosylated with neuraminidase and/or beta-galactosidase respectively. The efficacy of deglycosylations were assessed by peanut agglutinin (PNA) and vicia villosa lectin (VVL). Binding capacties of differently glycosylated IgA1 to HUVEC were evaluated by flow cytometry.
Results: IgA1 could bind to HUVEC and the binding capacities of IgA1, DesIgA1 and Des/DeGalIgA1 were expressed by median fluorescence intensity (MFI) and they were 2.67+/-0.35, 4.62+/-1.09, 4.08+/-0.41 (IgA1 vs DesIgA1, P=0.015, IgA1 vs DesIgA1/DeGalIgA1, P=0.049, DesIgA1 vs DesIgA1/DeGalIgA1 , P>0.05), respectively.
Conclusion: IgA1 could bind to HUVEC directly, and the binding capacities of DesIgA1 and Des/DeGalIgA1 to HUVEC were significantly higher than that of normal IgA1. Serum IgA1, especially deglycosylated IgA1, might play some role in vascular lesions of IgAN.